Human iPSC-derived hepatocytes in 2D and 3D suspension culture for cryopreservation and in vitro toxicity studies

被引:9
作者
Altmaier, Saskia [1 ]
Meiser, Ina [1 ]
Lemesre, Emilie [2 ]
Chanrion, Benjamin [2 ]
Steeg, Rachel [3 ]
Leonte, Lidia Elena [4 ,5 ]
Holst, Bjorn [4 ]
Nielsen, Boye Schnack [4 ]
Clausen, Christian [4 ]
Schmidt, Katharina [1 ]
Vinggaard, Anne Marie [5 ]
Zimmermann, Heiko [1 ,6 ,7 ]
Neubauer, Julia Christiane [1 ]
Rasmussen, Mikkel Aabech [4 ]
机构
[1] Fraunhofer Inst Biomed Engn, IBMT, Joseph-von-Fraunhofer-Weg 1, D-66820 Sulzbach, Germany
[2] Inst Rech SERVIER, Chemin Ronde 125, F-78290 Croissy Sur Seine, France
[3] Fraunhofer UK Res Ltd, Technol & Innovat Ctr, George St 99, Glasgow G11RD, Scotland
[4] Bioneer A S, Kogle 2, DK-2970 Horsholm, Denmark
[5] Tech Univ Denmark, Natl Food Inst, Kemitorvet Bygning 202, DK-2800 Lyngby, Denmark
[6] Saarland Univ, Dept Mol & Cellular Biotechnol, Dept Nanotechnol, D-66123 Saarbrucken, Germany
[7] Univ Catolica Norte, Fac Ciencias Mar, Coquimbo, Chile
基金
欧盟地平线“2020”;
关键词
Human induced pluripotent stem cells; Hepatocytes; In vitro toxicology; Nanoluciferase reporter; Miniaturization; Hepatic organoids; Cryopreservation; Upscaling; PLURIPOTENT STEM-CELLS; INTRACELLULAR ICE FORMATION; SMOOTH-MUSCLE; VIABILITY; TISSUE; VITRIFICATION; MOUSE; DIFFERENTIATION; EXPRESSION; MECHANISM;
D O I
10.1016/j.reprotox.2022.05.005
中图分类号
Q [生物科学];
学科分类号
07 ; 0710 ; 09 ;
摘要
Hepatocytes are of special interest in biomedical research for disease modelling, drug screening and in vitro toxicology. Human induced pluripotent stem cell (hiPSC)-derived hepatocytes could complement primary human hepatocytes due to their capability for large-scale expansion. In this study, we present an optimized protocol for the generation of hepatocyte-like cells (HLCs) from hiPSC in monolayer (2D) and suspension culture (3D) for production of organoids. A protocol was initially optimized in 2D using a gene edited CYP3A4 Nanoluciferase reporter hiPSC line for monitoring the maturity of HLCs and cryopreservation of definitive endoderm (DE) cells. The protocol was optimized for microwell cultures for high-throughput screening to allow for a sensitive and fast readout of drug toxicity. To meet the increasing demand of hepatic cells in biomedical research, the differentiation process was furthermore translated to scalable suspension-based bioreactors for establishment of hepatic organoids. In pilot studies, the technical settings have been optimized by adjusting the initial seeding density, rotation speed, inoculation time, and medium viscosity to produce homogeneous hepatic organoids and to maximize the biomass yield (230 organoids/ml). To speed up the production process, cryopreservation approaches for the controlled freezing of organoids were analysed with respect to cell recovery and marker expression. The results showed that cryopreserved organoids maintained their phenotype only when derived from hepatocyte progenitors (HPs) at day 8 but not from more mature stages. The establishment of robust protocols for the production of large batches of hepatocytes and hepatic organoids could substantially boost their use in biomedical and toxicology studies.
引用
收藏
页码:68 / 80
页数:13
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